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Direct STR typing from bullet casings

FSI Genetics Supplement Series, 2017

Study Design

Addressed Question

evaluation of direct PCR as an alternative method to STR typing from bullet casings

Activity Context

Shooting

Category

PersistenceRecovery

Specifications

Direct PCRPersistence with Firing / Explosion

Variables of Interest

extraction vs. Direct PCRbullet type

Stringency of Control

Controlled

Number of Individuals

10

Replicates per Individual and Condition

2

Nucleic Acid

DNA

Bodily Origin

skin (hands)

Depositor & Contact

Depositor Characteristics

N/A

Criteria for Shedder Status

N/A

Previous Activities

N/A

Contact Scenario

handling of bullets - firing - sampling - randomization into direct PCR vs conventional PCR groups

Primary Substrate

Primary Substrate Type

cartridges: 9mm, 5.56mm, 7.62mm bullets

Primary Substrate Material

N/A

Deposit

handling for 15s in each hand

Delay

N/A

Secondary Substrate

Secondary Substrate Type

N/A

Secondary Substrate Material

N/A

Secondary Substrate Contact

N/A

Further Transfer

N/A

Sampling

Background DNA on Sampled Surface

N/A

Sampling Time

direct

Persistence

firing all bullets

Sampling Method

single swabbing, EO cotton swab moistened with PBS

Sampling Area

outer ammunition surface

Laboratory Analysis

Extraction

Promega IQ kit or direct PCR

DNA Quantification

Quantifiler kit or not quantified

Input for Profiling

0.5 ng or max. 5 µl extract, direct PCR: ten 1mm^2 pieces from swab

Profiling

Identifiler Plus kit, ABI 3130, GeneMapper

Reference Samples

N/A

Profile Interpretation and Mixture Analysis

N/A

RNA Data Interpretation

N/A

Results

DNA Quantity

N/A

Profile Quality

mostly incomplete, not useful profiles

Parameter Used for Comparison

number of alleles detected

Summary of Results

number of alleles recovered using the direct PCR protocol does not differ statistically from conventional extraction STR typing protocol (median: 3.0-3.5 alleles); (assumption: more DNA is added in the directPCR approach, but so are more metal ions from casings and GSR inhibiting PCR); direct PCR method is quicker and cheaper

Raised Questions

N/A

Cautionary Remarks

presence of inhibitors in direct PCR reaction not experimentally confirmed; n.a. whether profiles were attributable to depositor